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Direct visualization of G-quadruplexes in DNA using atomic force microscopy.

机译:使用原子力显微镜直接观察DNA中的G-四链体。

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The formation of G-quadruplexes in G-rich regions of DNA is believed to affect DNA transcription and replication. However, it is currently unclear how this formation occurs in the presence of a complementary strand. We have used atomic force microscopy (AFM) to image stable RNA/DNA hybrid loops generated by transcription of the plasmid pPH600, which contains a 604-bp fragment of the murine immunoglobulin Sd3 switch region. We show that the non-RNA-containing portion folds into G-quadruplexes, consistent with computational predictions. We also show that hybrid formation prevents further transcription from occurring, implying a regulatory role. After in vitro transcription, almost all (93%) of the plasmids had an asymmetric loop, a large asymmetric blob or a spur-like projection at the appropriate position on the DNA contour. The loops disappeared following treatment of the transcribed plasmid with RNase H, which removes mRNA hybridized with the template strand. Replacement of K in the transcription buffer with either Na or Li caused a reduction in the percentage of plasmids containing loops, blobs or spurs, consistent with the known effects of monovalent cations on G-quadruplex stability. The minimal sample preparation required for AFM imaging has permitted direct observation of the structural changes resulting from G-quadruplex formation.
机译:据信在富含G的DNA区域中形成G-四链体会影响DNA的转录和复制。然而,目前尚不清楚在互补链的存在下该形成如何发生。我们已经使用原子力显微镜(AFM)来成像由质粒pPH600的转录产生的稳定的RNA / DNA杂交环,该质粒包含鼠免疫球蛋白Sd3开关区域的604-bp片段。我们表明,不包含RNA的部分折叠成G四联体,与计算预测一致。我们还表明,杂合体的形成阻止了进一步转录的发生,这暗示着调节作用。体外转录后,几乎所有质粒(93%)在DNA轮廓上的适当位置均具有不对称环,较大的不对称斑点或类似马刺的突起。用RNase H处理转录的质粒后,环消失,该酶去除了与模板链杂交的mRNA。用Na或Li替换转录缓冲液中的K会导致含有环,斑点或刺的质粒百分比降低,这与一价阳离子对G-四链体稳定性的已知作用相一致。原子力显微镜成像所需的最少样品制备已允许直接观察由G四链体形成引起的结构变化。

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